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鉴定出一种人类雌激素受体α(hER-α)的新亚型,它由不同的转录本编码,并且能够抑制hER-α激活功能1。

Identification of a new isoform of the human estrogen receptor-alpha (hER-alpha) that is encoded by distinct transcripts and that is able to repress hER-alpha activation function 1.

作者信息

Flouriot G, Brand H, Denger S, Metivier R, Kos M, Reid G, Sonntag-Buck V, Gannon F

机构信息

EMBL, Meyerhofstrabetae 1, D-69117 Heidelberg, Germany and Endocrinologie Moléculaire de la Reproduction, UPRES-A CNRS 6026, Campus de Beaulieu, 35042 Rennes cedex, France.

出版信息

EMBO J. 2000 Sep 1;19(17):4688-700. doi: 10.1093/emboj/19.17.4688.

Abstract

A new isoform of the human estrogen receptor-alpha (hER-alpha) has been identified and characterized. This 46 kDa isoform (hERalpha46) lacks the N-terminal 173 amino acids present in the previously characterized 66 kDa isoform (hERalpha66). hERalpha46 is encoded by a new class of hER-alpha transcript that lacks the first coding exon (exon 1A) of the ER-alpha gene. We demonstrated that these Delta1A hER-alpha transcripts originate from the E and F hER-alpha promoters and are produced by the splicing of exon 1E directly to exon 2. Functional analysis of hERalpha46 showed that, in a cell context sensitive to the transactivation function AF-2, this receptor is an effective ligand-inducible transcription factor. In contrast, hERalpha46 is a powerful inhibitor of hERalpha66 in a cell context where the transactivating function of AF-1 predominates over AF-2. The mechanisms by which the AF-1 dominant-negative action is exerted may involve heterodimeri zation of the two receptor isoforms and/or direct competition for the ER-alpha DNA-binding site. hERalpha66/hERalpha46 ratios change with the cell growth status of the breast carcinoma cell line MCF7, suggesting a role of hERalpha46 in cellular proliferation.

摘要

一种新的人雌激素受体α(hER-α)同工型已被鉴定和表征。这种46 kDa的同工型(hERα46)缺少先前表征的66 kDa同工型(hERα66)中存在的N端173个氨基酸。hERα46由一类新的hER-α转录本编码,该转录本缺少ER-α基因的第一个编码外显子(外显子1A)。我们证明这些Δ1A hER-α转录本源自E和F hER-α启动子,是通过外显子1E直接剪接到外显子2产生的。hERα46的功能分析表明,在对反式激活功能AF-2敏感的细胞环境中,该受体是一种有效的配体诱导型转录因子。相比之下,在AF-1的反式激活功能超过AF-2的细胞环境中,hERα46是hERα66的强力抑制剂。AF-1显性负性作用发挥的机制可能涉及两种受体同工型的异二聚化和/或对ER-α DNA结合位点的直接竞争。hERα66/hERα46比值随乳腺癌细胞系MCF7的细胞生长状态而变化,提示hERα46在细胞增殖中起作用。

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